Interaction des silicates tricalciques avec la pulpe dentaire : conséquences sur les étapes précoces de la régénération dentinaire

Laurent, Patrick

24 September 2012

Le coiffage pulpaire direct, dans des situations pathologiques critiques où la vitalité de la dent est menacée, vise à stimuler le potentiel de cicatrisation de la pulpe et induire une régénération dentinaire. Afin d'optimiser cette thérapeutique, le Laboratoire IMEB-ERT 30 a développé en partenariat avec la société SEPTODONT un nouveau matériau, le Biodentine™. Ce ciment, composé essentiellement de silicate tricalcique, possède des qualités physiques permettant son utilisation comme substitut dentinaire. Le premier objectif de notre travail a été d'évaluer les propriétés biologiques du Biodentine™ et ses interactions avec les cellules cibles en culture. La bioactivité du nouveau ciment a ensuite été étudiée à l'aide du modèle de culture de dents entières humaines ex vivo. Ce modèle expérimental original a été mis au point dans notre laboratoire et permet d'étudier les phases précoces de la régénération dentinaire lors du coiffage direct. Grâce à ce modèle, nous avons démontré l'activation, la prolifération et la migration de cellules progénitrices pulpaires périvasculaires en réponse à une lésion cavitaire profonde. Le coiffage direct avec les ciments de silicates tricalciques a induit la formation de foyers minéralisés à proximité de la lésion. La caractérisation moléculaire de ces foyers a montré qu'il s'agit d'une forme de dentine réparatrice synthétisée par des cellules odontoblast-like. Le deuxième objectif de notre travail a été d'étudier l'effet du nouveau biomatériau sur la sécrétion de certains facteurs de croissances, impliqués dans les phases précoces de la cicatrisation pulpaire, et de le comparer à celui d'autres matériaux de coiffage. / The objective of direct pulp capping is to stimulate the pulp healing potential and to induce dentin regeneration. This is of prime importance in critical pathologic situations compromising the tooth vitality. To improve the outcome of this treatment, the IMEB-ERT30 Laboratory, in collaboration with the SEPTODONT Company, has developed a new restorative material called Biodentine™. This cement, essentially composed of tricalcium silicates, has the required physical properties to be used as a dentin substitute. The first aim of this work was to evaluate the biological properties of Biodentine™ and its interactions with the target cells in cell culture. Then, the bioactivity of the new cement was studied using an entire human tooth culture model ex vivo. This original experimental model, developed in our Laboratory, is suitable in studying the early steps of dentin regeneration after direct pulp capping. With this model, we demonstrated the activation, proliferation, and migration of perivascular pulpal progenitor cells in response to pulp injury. The direct pulp capping with tricalcium silicate cements induced mineral foci formation in the vicinity of the pulp lesion. Molecular characterization of these foci confirmed it was of a reparative dentin type produced by odontoblast-like cells. The second objective of our work was to study the effect of the new cement on the secretion of some growth factors involved in the early steps of pulp wound healing, and compare it to that of other pulp capping materials. The results demonstrated an up-regulation of b-FGF, VEGF and PDGF-AB secretion in response to the target cells injuries, suggesting a stimulation of angiogenesis.

Fibroblastes pulpaires

Angiogenèse

Coiffage pulpaire

Facteurs de croissance

Régénération dentinaire

Pulp fibroblast

Angiogenesis

Progenitor mesenchymal cells

Pulp capping

Growth factors

Dentin regeneration.

"Resposta de fibroblastos de polpa humanos submetidos a substâncias liberadas por capeadores pulpares diretos" / Human pulp fibroblasts response to substances leached from direct pulp capping materials

Cavalcanti, Bruno das Neves

04 February 2004

Cavalcanti, BN. Resposta de fibroblastos de polpa humanos frente a substâncias liberadas por capeadores pulpares diretos [Tese de Doutorado]. São Paulo: Faculdade de Odontologia da USP; 2003. RESUMO O objetivo do presente estudo foi o de avaliar os efeitos citotóxicos de substâncias liberadas durante a aplicação de materiais utilizados em capeamento pulpar direto, sobre fibroblastos de polpa dentária humana. Utilizou-se para o experimento meios condicionados pelas substâncias a serem testadas, divididas nos grupos a seguir: grupo I: controle (meio de cultivo sem condicionamento); grupo II: cimento de hidróxido de cálcio; grupo III: adesivo dentinário; grupo IV: ácido ortofosfórico a 37%. O condicionamento foi realizado, colocando-se meio de cultivo fresco sobre os materiais de modo que a presa (grupo II), polimerização (grupo III) ou o contato direto (grupo IV) liberassem substâncias para esse meio de cultivo. Esse meio era colocado sobre as células durante todo o experimento, excetuando-se o grupo IV, onde o contato foi feito por um período de 15 segundos, conforme recomendações clínicas. Posteriormente foram realizadas contagens em hemocitômetro pelo método de exclusão por azul de Trypan, que cora somente as células mortas. As contagens foram realizadas em períodos de 0, 6, 12 e 24 horas para o experimento de viabilidade celular (curto prazo), onde se avaliou o percentual de células vivas sobre o total de células, e em períodos de 1, 3, 5 e 7 dias para o experimento de sobrevivência celular, no qual se avaliou o número absoluto de células vivas. Observou-se que as substâncias liberadas pelo adesivo dentinário são citotóxicas em qualquer período, diminuindo consideravelmente a viabilidade celular e afetando suas curvas de crescimento. Aquelas liberadas pelo ácido ortofosfórico a 37% provocam diminuição da viabilidade somente nos primeiros momentos do contato com as células, enquanto as substâncias liberadas durante a presa do hidróxido de cálcio não são citotóxicas em nenhum momento. / The purpose of the present study was to evaluate the cytotoxic effects of substances leached during the use of direct pulp capping materials, on human pulp fibroblasts. There were used cell culture mediums conditioned by the test materials, as follows: group I: control (fresh medium without conditioning); group II: calcium hydroxide cement; group III: bonding system; group IV: 37% orthophosphoric acid. The medium conditioning was made, pouring the fresh conditioning medium on the materials, in order that its setting (group II), polymerization (group III) or the direct contact (group IV) would be able to leach substances to this culture medium. These conditioned mediums were put on the cells for the entire experiment, excepting the group IV, in which the mediums were put in contact with the cells for 15 seconds, following clinical recommendations. Cell counting was performed in hemocytometer, using the Trypan blue exclusion method, which mark only the dead cells. These counting was made at experimental times of 0, 6, 12 and 24 hours for the cell viability assay (short term), where it is evaluated the percentage of live cells on the total number of cells, and at experimental times of 1, 3, 5 and 7 days for the survival assay, in which is evaluated the absolute number of live cells. It was observed that the substances leached by the bonding system are cytotoxic at all experimental times, decreasing significantly the cell viability and affecting its growing rate. Those leached by the 37% orthophosphoric acid decreased the cell viability only at the first contact with the cells, and the substances leached during the setting of the calcium hydroxide cement are not cytotoxic.

Adesivos dentinários

Calcium hydroxide

Capeamento da polpa dentária

Dental pulp

Dental pulp capping

Dentin bonding system

Fibroblasto pulpar

Hidróxido de cálcio

Polpa dentária

Pulp fibroblast

"Resposta de fibroblastos de polpa humanos submetidos a substâncias liberadas por capeadores pulpares diretos" / Human pulp fibroblasts response to substances leached from direct pulp capping materials

Bruno das Neves Cavalcanti

04 February 2004

Cavalcanti, BN. Resposta de fibroblastos de polpa humanos frente a substâncias liberadas por capeadores pulpares diretos [Tese de Doutorado]. São Paulo: Faculdade de Odontologia da USP; 2003. RESUMO O objetivo do presente estudo foi o de avaliar os efeitos citotóxicos de substâncias liberadas durante a aplicação de materiais utilizados em capeamento pulpar direto, sobre fibroblastos de polpa dentária humana. Utilizou-se para o experimento meios condicionados pelas substâncias a serem testadas, divididas nos grupos a seguir: grupo I: controle (meio de cultivo sem condicionamento); grupo II: cimento de hidróxido de cálcio; grupo III: adesivo dentinário; grupo IV: ácido ortofosfórico a 37%. O condicionamento foi realizado, colocando-se meio de cultivo fresco sobre os materiais de modo que a presa (grupo II), polimerização (grupo III) ou o contato direto (grupo IV) liberassem substâncias para esse meio de cultivo. Esse meio era colocado sobre as células durante todo o experimento, excetuando-se o grupo IV, onde o contato foi feito por um período de 15 segundos, conforme recomendações clínicas. Posteriormente foram realizadas contagens em hemocitômetro pelo método de exclusão por azul de Trypan, que cora somente as células mortas. As contagens foram realizadas em períodos de 0, 6, 12 e 24 horas para o experimento de viabilidade celular (curto prazo), onde se avaliou o percentual de células vivas sobre o total de células, e em períodos de 1, 3, 5 e 7 dias para o experimento de sobrevivência celular, no qual se avaliou o número absoluto de células vivas. Observou-se que as substâncias liberadas pelo adesivo dentinário são citotóxicas em qualquer período, diminuindo consideravelmente a viabilidade celular e afetando suas curvas de crescimento. Aquelas liberadas pelo ácido ortofosfórico a 37% provocam diminuição da viabilidade somente nos primeiros momentos do contato com as células, enquanto as substâncias liberadas durante a presa do hidróxido de cálcio não são citotóxicas em nenhum momento. / The purpose of the present study was to evaluate the cytotoxic effects of substances leached during the use of direct pulp capping materials, on human pulp fibroblasts. There were used cell culture mediums conditioned by the test materials, as follows: group I: control (fresh medium without conditioning); group II: calcium hydroxide cement; group III: bonding system; group IV: 37% orthophosphoric acid. The medium conditioning was made, pouring the fresh conditioning medium on the materials, in order that its setting (group II), polymerization (group III) or the direct contact (group IV) would be able to leach substances to this culture medium. These conditioned mediums were put on the cells for the entire experiment, excepting the group IV, in which the mediums were put in contact with the cells for 15 seconds, following clinical recommendations. Cell counting was performed in hemocytometer, using the Trypan blue exclusion method, which mark only the dead cells. These counting was made at experimental times of 0, 6, 12 and 24 hours for the cell viability assay (short term), where it is evaluated the percentage of live cells on the total number of cells, and at experimental times of 1, 3, 5 and 7 days for the survival assay, in which is evaluated the absolute number of live cells. It was observed that the substances leached by the bonding system are cytotoxic at all experimental times, decreasing significantly the cell viability and affecting its growing rate. Those leached by the 37% orthophosphoric acid decreased the cell viability only at the first contact with the cells, and the substances leached during the setting of the calcium hydroxide cement are not cytotoxic.

Adesivos dentinários

Capeamento da polpa dentária

Fibroblasto pulpar

Hidróxido de cálcio

Polpa dentária

Calcium hydroxide

Dental pulp

Dental pulp capping

Dentin bonding system

Pulp fibroblast